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通过光刺激或化学刺激双重激活 cAMP 产生。

Dual Activation of cAMP Production Through Photostimulation or Chemical Stimulation.

机构信息

Department of Pharmacology and Chemical Biology, University of Pittsburgh, Pittsburgh, PA, USA.

Molecular Pharmacology Training Program, University of Pittsburgh, Pittsburgh, PA, USA.

出版信息

Methods Mol Biol. 2020;2173:201-216. doi: 10.1007/978-1-0716-0755-8_14.

Abstract

cAMP is a crucial mediator of multiple cell signaling pathways. This cyclic nucleotide requires strict spatiotemporal control for effective function. Light-activated proteins have become a powerful tool to study signaling kinetics due to having quick on/off rates and minimal off-target effects. The photoactivated adenylyl cyclase from Beggiatoa (bPAC) produces cAMP rapidly upon stimulation with blue light. However, light delivery is not always feasible, especially in vivo. Hence, we created a luminescence-activated cyclase by fusing bPAC with nanoluciferase (nLuc) to allow chemical activation of cAMP activity. This dual-activated adenylyl cyclase can be stimulated using short bursts of light or long-term chemical activation with furimazine and other related luciferins. Together these can be used to mimic transient, chronic, and oscillating patterns of cAMP signaling. Moreover, when coupled to compartment-specific targeting domains, these reagents provide a new powerful tool for cAMP spatiotemporal dynamic studies. Here, we describe detailed methods for working with bPAC-nLuc in mammalian cells, stimulating cAMP production with light and luciferins, and measuring total cAMP accumulation.

摘要

cAMP 是多种细胞信号通路的关键介质。这种环状核苷酸需要严格的时空控制才能发挥有效功能。由于具有快速的开启/关闭速率和最小的脱靶效应,光激活蛋白已成为研究信号转导动力学的有力工具。来自 Beggiatoa 的光激活腺苷酸环化酶(bPAC)在受到蓝光刺激时会迅速产生 cAMP。然而,光传递并不总是可行的,特别是在体内。因此,我们通过将 bPAC 与纳米荧光素酶(nLuc)融合,创建了一种发光激活的环化酶,以允许化学激活 cAMP 活性。这种双激活的腺苷酸环化酶可以使用短脉冲的光或 Furimazine 和其他相关荧光素的长期化学激活来刺激。这些可以一起用于模拟 cAMP 信号的瞬时、慢性和振荡模式。此外,当与特定于隔室的靶向结构域结合时,这些试剂为 cAMP 时空动态研究提供了一种新的强大工具。在这里,我们描述了在哺乳动物细胞中使用 bPAC-nLuc 的详细方法,用光和荧光素刺激 cAMP 的产生,并测量总 cAMP 积累。

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